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基于PCR-CRSIPR/Cas12a的DNMT3A R882H/C可视化检测方法

蒋清杨孙如美缪夏萍范喜杰张浩名夏银骁李凯敏陈涛

分子影像学杂志2025，Vol.48Issue(5)：589-596,8.

分子影像学杂志2025，Vol.48Issue(5)：589-596,8.DOI:10.12122/j.issn.1674-4500.2025.05.09

基于PCR-CRSIPR/Cas12a的DNMT3A R882H/C可视化检测方法

Establishment of a PCR-CRISPR/Cas12a-based visual detection method for DNMT3A R882H/C

蒋清杨 ¹孙如美 ²缪夏萍 ²范喜杰 ²张浩名 ³夏银骁 ¹李凯敏 ⁴陈涛⁵

作者信息

1. 广州医科大学金域检验学院,广东广州 510182
2. 广州市金域转化医学研究院有限公司,广东广州 510220
3. 广州医科大学金域检验学院,广东广州 510182||广州市金域转化医学研究院有限公司,广东广州 510220
4. 烟台毓璜顶医院,山东烟台 264000
5. 广州医科大学金域检验学院,广东广州 510182||广州市金域转化医学研究院有限公司,广东广州 510220||广州金域医学检验中心有限公司感染性疾病检测中心,广东广州 510220
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摘要

Abstract

Objective To develop a DNMT3A R882H(c.2645G>A)and R882C(c.2644C>T)visual detection system based on polymerase chain reaction(PCR)and clustered regularly interspaced short palindromic repeats(CRISPR)with their associated protein(Cas12a).Methods Thirty-four bone marrow samples from patients suspected of acute myeloid leukemia were collected at a hospital from September 2023 to September 2024.The specific amplification primers and CRISPR RNA(crRNA)for the PCR-Cas12a nucleic acid detection system were designed to target the DNMT3A R882H/C mutation sites.Primer pairs with optimal amplification performance were selected using agarose gel electrophoresis,and the fluorescence intensity generated by Cas12a protein cleavage of nearby fluorescent probes was used to identify the crRNA with the highest cleavage efficiency,based on the signal difference between mutant and wild-type sequences,to construct the PCR-Cas12a Nucleic Acid Detection System.Wild-type human genomic DNA and DNMT3A R882H/C mutant plasmids were mixed in varying ratios to simulate different mutation frequencies and assess the detection limit of PCR-Cas12a.Finally,clinical samples validated for DNMT3A R882H/C mutations by high-throughput sequencing were tested using PCR-Cas12a to evaluate methodological consistency and resistance to interference.Results The PCR-Cas12a nucleic acid visual detection system effectively detected DNMT3A R882H/C mutations in clinical samples with mutation frequencies as low as 1%.Conclusion This study established a visual detection method for DNMT3A R882H/C mutations by combining PCR with CRISPR-Cas12a technology,which is rapid,specific,and sensitive,providing robust support for the prognostic assessment of acute myeloid leukemia.

关键词

CRISPR/Cas12a/DNMT3A R882H/DNMT3A R882C/急性髓系白血病/可视化检测

Key words

CRISPR/Cas12a/DNMT3A R882H/DNMT3A R882C/acute myeloid leukemia/visual detection

引用本文复制引用

蒋清杨,孙如美,缪夏萍,范喜杰,张浩名,夏银骁,李凯敏,陈涛..基于PCR-CRSIPR/Cas12a的DNMT3A R882H/C可视化检测方法[J].分子影像学杂志,2025,48(5):589-596,8.

基金项目

市校(院)企联合资助专题(2023A03J0542) （院）

分子影像学杂志

ISSN：1674-4500

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